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srf2fastq(1)			 Staden io_lib			  srf2fastq(1)

NAME
       srf2fastq - Converts SRF files to Sanger fastq format

SYNOPSIS
       srf2fastq  [options] srf_archive ...

DESCRIPTION
       srf2fastq  extracts  sequences  and  qualities from one or more SRF ar‐
       chives and writes them in Sanger fastq format to stdout.

       Note that Illumina also have a fastq format (used in the GERALD	direc‐
       tories)	which  differs	slightly in the use of log-odds scores for the
       quality values. The format described  here  is  using  the  traditional
       Phred style of quality encoding.

OPTIONS
       -c     Outputs  calibrated  confidence  values using the ZTR CNF1 chunk
	      type for a single quality per base. Without this use the	origi‐
	      nal  Illumina  _prb.txt  files consisting of four quality values
	      per base, stored in the ZTR CNF4 chunks.

       -C     Masks out sequences tagged as bad quality.

       -s root
	      Generates files on disk with filenames starting root,  one  file
	      per  non-explicit	 element  in  the SRF/ZTR region (REGN) chunk.
	      Typically this results in two files for  paired  end  runs.  The
	      filename	suffixes  come from the names listed in the SRF region
	      chunks.  This option conflicts with the -S parameter.

       -S     Splits sequences	into  regions,	but  sequentially  lists  each
	      sequence region to stdout instead of splitting to separate files
	      on disk. This option conflicts with the -s parameter.

       -n     When using -s the filename suffixes are simply numbered  (start‐
	      ing  with 1) instead of using the names listed in the SRF region
	      chunks.

       -a     Appends region index to the sequence names. Ie generate "name/1"
	      and "name/2" for a paired read.

       -e     Include  any explicit sequence (ZTR region chunk of type 'E') in
	      the sequence output. The explicit sequence is also  included  in
	      the quality line too. Currently this is utilised by ABI SOLiD to
	      store the last base of the primer.

       -r region list
	      Reverse complements the sequence and reverses the quality values
	      for  all	regions	 in the region list. This is a comma separated
	      list of integer values enumerating the regions, starting from 1.
	      Note that this option only works when either -s or -S are speci‐
	      fied.

EXAMPLES
       To extract only the good quality sequences from all srf	files  in  the
       current directory using calibrated confidence values (if available).

	   srf2fastq -c -C *.srf > runX.fastq

       To  extract  a  paired  end  run into two separate files with sequences
       named name/1 and name/2.

	   srf2fastq -s runX -a -n runX.srf

       To extract a paired end run as a single file, alternating  forward  and
       reverse sequences, with the second read being reverse complemented.

	   srf2fastq -S -r 2 runX.srf > runX.fastq

AUTHOR
       James Bonfield, Steven Leonard - Wellcome Trust Sanger Institute

				  December 10			  srf2fastq(1)

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